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Complementation of methylation deficiency in embryonic stem cells by a DNA methyltransferase minigene

机译:胚胎干细胞甲基化缺乏症的补充 通过DNA甲基转移酶微基因

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摘要

Previous attempts to express functional DNA cytosine methyltransferase (EC 2.1.1.37) in cells transfected with the available Dnmt cDNAs have met with little or no success. We show that the published Dnmt sequence encodes an amino terminal-truncated protein that is tolerated only at very low levels when stably expressed in embryonic stem cells. Normal expression levels were, however, obtained with constructs containing a continuation of an ORF with a coding capacity of up to 171 amino acids upstream of the previously defined start site. The protein encoded by these constructs comigrated in SDS/PAGE with the endogenous enzyme and restored methylation activity in transfected cells. This was shown by functional rescue of Dnmt mutant embryonic stem cells that contain highly demethylated genomic DNA and fail to differentiate normally. When transfected with the minigene construct, the genomic DNA became remethylated and the cells regained the capacity to form teratomas that displayed a wide variety of differentiated cell types. Our results define an amino-terminal domain of the mammalian MTase that is crucial for stable expression and function in vivo.
机译:先前尝试在用可用Dnmt cDNA转染的细胞中表达功能性DNA胞嘧啶甲基转移酶(EC 2.1.1.37)的尝试很少成功,甚至没有成功。我们表明,已发布的Dnmt序列编码在胚胎干细胞中稳定表达时仅能以非常低的水平耐受的氨基末端截短蛋白。然而,用含有ORF的连续体的构建体获得了正常表达水平,该ORF具有在先前定义的起始位点上游的至多171个氨基酸的编码能力。这些构建体编码的蛋白质在SDS / PAGE中与内源酶竞争,并在转染的细胞中恢复了甲基化活性。 Dnmt突变型胚胎干细胞的功能性抢救显示了这一点,该干细胞含有高度去甲基化的基因组DNA,无法正常分化。当用小基因构建体转染时,基因组DNA被重新甲基化,细胞重新获得形成畸胎瘤的能力,畸胎瘤显示出多种分化的细胞类型。我们的结果定义了哺乳动物MTase的氨基末端结构域, 对于体内稳定表达和功能至关重要。

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